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Previous Article | Next Article
The Journal of Neuroscience, July 1, 1999, 19(13):5409-5419
Expression of the Striatal DARPP-32/ARPP-21 Phenotype in GABAergic Neurons Requires Neurotrophins In Vivo and In Vitro
Sanja Ivkovic and Michelle E. Ehrlich The Nathan Kline Institute for Psychiatric Research, Orangeburg, New York 10962
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
The medium spiny neuron (MSN) is the major output neuron of the caudate nucleus and uses GABA as its primary neurotransmitter. A majority of MSNs coexpress DARPP-32 and ARPP-21, two dopamine and cyclic AMP-regulated phosphoproteins, and most of the matrix neurons express calbindin. DARPP-32 is the most commonly used MSN marker, but previous attempts to express this gene in vitro have failed. In this study we found that DARPP-32 is expressed in <12% of E13- or E17-derived striatal neurons when they are grown in defined media at high or low density in serum, dopamine, or Neurobasal/N2 (Life Technologies), and ARPP-21 is expressed in <1%. The percentage increases to 25% for DARPP-32 and 10% for ARPP-21 when the same cells are grown in Neurobasal/B27 (Life Technologies) for 7 d. After growth in Neurobasal/B27 plus brain-derived neurotrophic factor (BDNF) for 7 d, E13-derived MSNs are 53.7% DARPP-32-positive and 29.0% ARPP-21-positive; E17-derived MSNs are 66.8% DARPP-32-positive and 51.5% ARPP-21-positive. The percentage of calbindin-positive neurons also is increased under these conditions. Finally, ARPP-21 expression is reduced in mice with a targeted deletion of the BDNF gene. We conclude that BDNF is required for the maturation of a large subset of patch and matrix MSNs in vivo and in vitro. In addition, we introduce a culture system in which highly differentiated MSNs may be generated, maintained, and studied.
Key words: striatum; lateral ganglionic eminence; brain-derived neurotrophic factor; DARPP-32; ARPP-21; calbindin
INTRODUCTION
Neuronal phenotypes are regulated by cell intrinsic and extrinsic factors, but most of the details of the molecular specification of phenotype remain unknown. The caudate nucleus ("striatum") is a useful model for experimental investigation of neuronal differentiation. It is composed of cells that arise primarily from the lateral ganglionic eminence (LGE) (Deacon et al., 1994
; Nakao et al., 1994b
Transplant paradigms suggest that many undifferentiated progenitor cells in the LGE are committed to the MSN phenotype. We demonstrated that, when dissociated rat E14 LGE cells are transplanted into the embryonic brain, most of the surviving neurons reaggregate after migration into the parenchyma. Many of these mitotic, clustered cells differentiate according to their site of origin and ultimately express DARPP-32 and ARPP-21 (Magrassi et al., 1998
On the basis of the transplant data, it was anticipated that a large percentage of dissociated progenitor and postmitotic LGE neurons would develop the DARPP-32 phenotype in vitro. Surprisingly, however, under the conditions used to date, <5% of the LGE-derived neurons express DARPP-32 after 1 DIV in defined media (Nakao et al., 1994a
In this study we systematically identify the culture conditions under which a majority of MSNs survive but do not phenotypically mature. For the first time we identify basal conditions in which the addition of exogenous neurotrophins leads to the expression of DARPP-32, ARPP-21, and calbindin in up to 70% of the surviving neurons. These data provide definitive evidence that neurotrophins promote the maturation of MSNs. Also, this culture system should provide a valuable approach to the study of isolated, phenotypically mature MSNs.
MATERIALS AND METHODS
Cell culture. Timed-mated Swiss-Webster mouse dams were anesthetized with pentobarbital (day of plug = E0-E0.5), and the embryos were removed. The meninges were removed, and the LGE (E13 and E15) or the striatum [E17-postnatal day 0 (P0)] was isolated. The tissue was minced with a scalpel blade and incubated in Ca2+/Mg2+-free HBSS (CMF-HBSS) for 8 min at 37°C in a clinical rotator (40 rpm). The incubation mixture was replaced with 0.01% trypsin/CMF-HBSS (E13 and E15) or 2 mg/ml papain (E17 and P0) (Sigma, St. Louis, MO) in CMF-HBSS, incubated for 8 min, and rinsed twice in Leibovitz's medium (L-15; Life Technologies, Gaithersburg, MD). Then it was suspended in DMEM with 10% fetal calf serum (FCS), glucose (6 mg/ml), glutamine (1.4 mM), and penicillin/streptomycin (100 U/ml). This medium will be referred to as "RF." Cells were triturated through a glass bore pipette and plated onto Lab-Tek culture dishes coated with polymerized polyornithine (0.1 mg/ml in 15 mM borate buffer, pH 8.4), layered with merosin (2.5 µg/ml) (Life Technologies), and air-dried. Cell death was quantitated by trypan blue exclusion, and the neurons were not plated unless >95% excluded the dye after the dissociation procedure. Then 1 hr later the medium was replaced with defined medium (DM), a mixture of DMEM and F12 with additional insulin, transferrin, selenium (Collaborative Research ITS+ premix, Bedford, MA), and glucose and glutamine, as above, or with Neurobasal/N2 (Life Technologies) or with Neurobasal/B27 (Life Technologies), all with penicillin/streptomycin (100 U/ml). For specific experiments as noted, cells were maintained in serum. In all cases, media, including all additives, were changed every 48 hr. Dose-response curves for neurotrophins were performed for all media, with doses ranging from 1 to 1000 ng/ml. For BDNF, NT-3, and NT-4/5 the maximum responsivity was always seen at 50-100 ng/ml (data not shown). Therefore, unless otherwise indicated, all experiments were performed at 100 ng/ml. Antimitotic agents are added only where indicated because glial growth in B27 is extremely limited (Brewer et al., 1993
Immunocytochemistry. Prenatal whole brains or cultures were immersion-fixed in 4% paraformaldehyde in 0.1 M phosphate buffer, pH 7.4, whereas P0 brains were fixed by transcardial perfusion. Then tissue sections (30 µm) or cultures were processed with the appropriate primary and secondary antibodies by using the immunoperoxidase/ABC method (Vector Laboratories Elite Vectastain, Burlingame, CA). Neuronal purity was assessed by staining parallel cultures with neuron-specific enolase (Polyscience, 1:5000). The mouse monoclonal DARPP-32 (6a) and ARPP-21 (6a) antibodies (kindly provided by Drs. H. Hemmings and P. Greengard, Rockefeller University, NY) were used at 1:20,000 and 1:10,000 dilution, respectively. The anti-calbindin, anti-GABA (Sigma) and anti-phospho-ERK (New England Biolabs, Beverly, MA) antibodies were used at 1:1000 dilution. An examination of cultures immunostained with the DARPP-32 and calbindin antibodies revealed obvious, darkly staining neurons and some neurons that may have been stained lightly but were frequently difficult to distinguish from neurons that were unstained. Therefore, we counted only the darkly staining neurons. On the other hand, there was a clear distinction between all immunopositive and immunonegative neurons in cultures stained with the ARPP-21 antibody.
Western blot analysis. Proteins were derived from rapidly frozen cultures, eliminating the bias of selected field measurements. Total cellular protein was prepared according to the manufacturer's instructions (TRIzol; Life Technologies) or by lysis in boiling sample buffer (20% glycerol, 62.5 mM Tris-HCl, pH 6.9, 1% SDS, 5%
-mercaptoethanol, and 0.025% bromophenol blue), followed by sonication, 15 min of centrifugation, and recovery of the supernatants. Western blot analysis with 20-40 µg of protein was performed on 10% SDS-polyacrylamide gels. After transfer to nitrocellulose, the equal loading of proteins was confirmed by Ponceau stain because it was unknown as to whether various treatments would affect levels of "control" proteins, e.g., actin and tubulin. Western blot analysis with the DARPP-32 antibody was performed as previously described (Ehrlich et al., 1990
Quantification and statistical analysis. Total and/or representative neuronal number (enolase+, DARPP-32+, ARPP-21+, or calbindin+) were counted in sister cultures after immunocytochemical staining. Cell counting was performed at 10× or 20× in a premarked grid under phase-contrast. Total cell counts were performed on representative cultures to assess changes accurately in total cell number. To demonstrate that the counting of representative fields does not bias the results, we counted the total number of DARPP-32-positive cells in individual cultures. From E15-derived high-density cultures we counted three wells in DM (2124 ± 140) and three in BDNF (7434 ± 352) after 1 DIV, confirming our previous results from representative fields (Ivkovic et al., 1997
RESULTS
MSN survival in vitro is not accompanied by differentiation
We examined culture conditions that promote the survival of LGE-derived neurons to determine whether long-term survival in vitro is always accompanied by phenotypic differentiation. We were unable to use the system with which we had begun these studies (Ivkovic et al., 1997
E13 LGE-derived and E17 striatal neurons survived when they were grown at high density (1 × 106 cells/cm2) in DM or at low density in the presence of serum, dopamine, or in the commercial medium Neurobasal with the B27 additive (Life Technologies) (dal Toso et al., 1988
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Figure 1. BDNF promotes the expression of ARPP-21 in high-density cultures. A, E13-derived neurons plated at 1 × 106 cells/cm2 form large aggregates after 7 DIV but remain ARPP-21-negative. B, Treatment with BDNF (50 ng/ml) for the entire 7 DIV results in a marked increase in ARPP-21 immunopositivity. Magnification, 20×.
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Figure 2. Neurobasal/B27 promotes the differentiation of a subset of MSNs. The percentage of DARPP-32-positive neurons is increased in E13- and E17-derived low-density (1 × 105 cells/cm2) cultures grown in Neurobasal/B27 in the absence of exogenous growth factors relative to cultures grown at high density, in serum, or in the presence of dopamine. The percentage of DARPP-32-positive cells was calculated after 7 DIV, but the numbers in high-density (HD) cultures are approximate because of the difficulty of counting positive numbers of cells in aggregates. The percentage represents the average of fields from the center and the periphery of the cultures. The percentage in HD (1 × 106 cells/cm2) and in RF (defined medium plus 10% FCS) is greater than in DM plus dopamine (DA) (p < 0.01), and the percentage in Neurobasal/B27 is greater than in HD, RF, FCS or DA (p < 0.001).
Under all culture conditions that excluded serum, 90-95% of the surviving cells were positive for neuronal-specific enolase (Fig. 3A). This was true even in E17-derived cultures in Neurobasal/B27 in the absence of antimitotic agents. A majority of the neurons were GABA-positive (Fig. 3B) (Mizuno et al., 1994
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Figure 3. Representative E13- and E17-derived neurons cultured in Neurobasal/B27 and plated at 1 × 105 cells/cm2. A, E17-derived neurons, immunostained for neuron-specific enolase, after 1 DIV. B, E17-derived neurons, immunostained for GABA, after 1 DIV. C, D, E13-derived neurons stained for phospho-ERK in the absence (C) or presence (D) of BDNF (100 ng/ml) for 30 min. E-G, E17-derived neurons immunostained for DARPP-32 after 1 DIV in the absence of BDNF (E), after 7 DIV in the absence of BDNF (F), and after 7 DIV in the presence of BDNF (100 ng/ml) (G). Note the marked increase in soma size over time as induced by Neurobasal/B27 alone and further induced by the presence of BDNF. H, E13-derived neurons immunostained for ARPP-21 after 1 DIV in the presence of BDNF. I, J, E17-derived neurons stained for ARPP-21 after 7 DIV in the absence of BDNF (I) and after 7 DIV in the presence of BDNF (100 ng/ml) (J). K-M, E17-derived neurons immunostained for calbindin after 1 DIV in the absence of BDNF (K), 7 DIV in the absence of BDNF (L), and 7 DIV in the presence of BDNF (M). Magnification, 40×; scale bar, 30 µm.
We determined the percentage of DARPP-32- or ARPP-21-positive cells under all culture conditions at 7 DIV in the absence of neurotrophins (see Fig. 2). The percentage of DARPP-32-positive cells did not exceed 10% in high-density (HD) cultures and in low-density cultures grown in the presence of serum (RF) or dopamine (DA). In Neurobasal/B27 the percentage of DARPP-32-positive neurons exceeded 25% in both E13 and E17 cultures after 7 DIV in the absence of neurotrophins. ARPP-21 immunoreactivity, however, was detectable only in a very small percentage of neurons in Neurobasal/B27 cultures after 7 DIV and was very light (Fig. 3I). Approximately 50% of E13-derived cells survived for 7 DIV in Neurobasal/B27, and ~25% of E17-derived neurons survived, similar to that reported by Brewer (1995)
BDNF promotes appearance of the MSN phenotype in specific neuronal subsets
We next asked whether BDNF would stimulate medium spiny neuron progenitors grown in the presence of Neurobasal/B27 to express a mature phenotype, as defined by the expression of both DARPP-32 and ARPP-21. In the presence of BDNF (Table 1; Fig. 4A) the percentage of DARPP-32-positive neurons in E13 Neurobasal/B27 cultures rose from 8.6 to 20.6% after 1 DIV. In E17-derived cultures, it increased from 3.4 to 10.3% (Fig. 3E). After 7 DIV, E13 cultures in Neurobasal/B27 were 25% DARPP-32-positive; with the addition of exogenous BDNF for the entire 7 DIV, almost 54% were DARPP-32-positive. E17 cultures were almost 70% DARPP-32-positive in the presence of BDNF for 7 d but only 29% in its absence (Figs. 3F,G, 4A). In the presence of BDNF for 1 DIV, E13 and E17 cultures were 14.6 and 36% ARPP-21-positive (Figs. 3J, 4B), respectively. The percentage of ARPP-21-positive cells at 7 DIV in the presence of BDNF increased even further in both E13 and E17 cultures (Table 1). Therefore, BDNF is required for ARPP-21 expression in vitro even more so than that for DARPP-32.
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Table 1. Percentage of DARPP-32, ARPP-21, and calbindin-positive cells
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Figure 4. The percentage of DARPP-32- (A), ARPP-21- (B), and calbindin-positive (C) neurons increases in E13- and E17-derived cultures grown in the presence of BDNF. Neurons were cultured in Neurobasal/B27 (Control) alone for 1 or 7 d, in Neurobasal/B27 with the addition of 100 ng/ml BDNF for 1 or 7 d, or in Neurobasal/B27 for 6 d, followed by Neurobasal/B27 plus 100 ng/ml BDNF for day 7 (6+1). BDNF and 6+1 values were compared with control values in the same category. **All were significant at p < 0.001, except for E13/6+1 for DARPP-32 and E13/1 DIV for calbindin, which were not significant.
To eliminate potential bias from counting representative fields, we also performed Western analysis of DARPP-32 protein derived from scaled-up sister cultures. DARPP-32 protein was increased in E13 cultures in the presence of BDNF at both 1 and 7 DIV, as compared with cultures grown in Neurobasal/B27 alone (Fig. 5A). These blots also confirmed the increase in total DARPP-32 protein per culture in E15-, E18-, and P0-derived cultures after 1 DIV in the presence of BDNF (Fig. 5B).
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Figure 5. Western blot analyses of DARPP-32 protein in samples derived from whole cultures correlate with the numbers of percentage-positive neurons derived from selected field counts. A, Western blot analysis of DARPP-32 protein in E13-derived sister cultures maintained in Neurobasal/B27 with or without BDNF for 1 and 7 DIV. B, BDNF increases the amount of DARPP-32 protein in E13-, E15-, E18-, and P0-derived cultures after 1 DIV. CP, Control caudate putamen, 5 µg from adult mouse; N, Neurobasal/B27; B, Neurobasal/B27 plus BDNF, 100 ng/ml. C, NT-3 and NT-4/5, alone or in combination with BDNF, increase the amount of DARPP-32 protein in E13-derived cultures to the same extent as does BDNF alone. NFG does not increase DARPP-32 protein in sister cultures. The results with GDNF were somewhat variable, and this experiment is one in which GDNF increased the amount of DARPP-32 protein, but not the percentage of immunostained cells. All cultures included Neurobasal/B27 (NB). B, BDNF; N, NGF; 3, NT-3; 4, NT-4/5; G, GDNF; All, BDNF, NT-3, and NT-4/5, each at 25 ng/ml.
Neuronal survival rate at 1 DIV is >90% in E13 and E17 cultures in Neurobasal/B27 (Brewer, 1995
We therefore sought to determine whether exposure to BDNF for only 24 hr results in an increase in DARPP-32, ARPP-21, and calbindin expression in neurons that already have been in culture for 6 DIV (see Table 1; Fig. 4). In E13 cultures DARPP-32 immunopositivity tended to rise from 25 to almost 32%, but this increase did not reach statistical significance. In 6 DIV E17 cultures, however, the percentage of DARPP-32-positive cells rose from 29.3 to 47.3% (p < 0.001). For ARPP-21 immunopositivity the percentage in E13 cultures rose from 9.9 to 21% (p < 0.001) and, in E17 cultures, from 4.4 to 22.3% (p < 0.001) in the presence of BDNF. Calbindin immunopositivity doubled (p < 0.001), reaching the same level as in cultures that were in BDNF for the entire 7 d. The fact that DARPP-32 and ARPP-21 immunopositivity did not reach the same levels as achieved after a full 7 DIV in the presence of growth factor may indicate that the maturation process and successive gene expression require >24 hr, depending on the stage of the cell. It is also possible that there is a subset of progenitor cells that are induced to proliferate and express DARPP-32 and ARPP-21, but not calbindin. If this were the case, however, there likely would be a significant increase in total neuronal number in the presence of BDNF, which did not occur. Because BDNF does not have a measurable mitotic effect on a mix of striatal progenitors (Ventimiglia et al., 1995
Previous studies examining the DARPP-32 phenotype in MSNs in dissociated culture after exposure to neurotrophins used a system in which the cells remained in serum for 24 hr (Nakao et al., 1994a
Finally, we sought to determine the specificity of the response to BDNF. We first investigated whether all neurons in LGE-derived cultures that are BDNF-responsive express DARPP-32 in its presence. In E13-derived cultures >90% of the neurons at 1 DIV are responsive to BDNF, as determined by the immunodetection of phospho-ERK after 30 min of exposure to BDNF (see Fig. 3C,D). After 24 hr of exposure to BDNF, however, only 20.6% of the neurons are DARPP-32-positive and, after 7 DIV, 53.7%. Therefore, expression of DARPP-32 may require BDNF and, in a subset of MSNs, other unidentified factors. Cultures from the lateral ganglionic eminence also contain GABAergic cells that in vivo ultimately populate the cortex (Anderson et al., 1997b
E13-Derived and E17-derived neurons represent different striatal compartments, both regulated by BDNF
When we extrapolate to the mouse from studies performed in the rat (van der Kooy and Fishell, 1987
We hypothesized that E13-derived cultures should contain fewer calbindin-positive cells than E17-derived cultures, particularly at 1 DIV. E17-derived cultures would be expected to contain most of the patch neurons (if they survived the dissociation and plating procedure) and a majority of matrix neurons, as are present in the adult striatum. We found that, in Neurobasal/B27 without exogenous growth factors, E13 cultures were <3% calbindin-positive at 1 DIV and 17% positive at 7 DIV. E17 cultures were almost 19% calbindin-positive at 1 DIV and almost 32% positive at 7 DIV (see Fig. 3K-M). In the presence of BDNF for 1 DIV, the number in the E13 cultures did not increase, whereas it almost doubled in E17 cultures (see Fig. 4C). These numbers are in contrast to the percentage of DARPP-32-positive neurons, which is higher in E13 than in E17 at 1 DIV. These data imply that the cultures are not distinguished solely on the basis of their overall well being and/or maturity. By 7 DIV in the presence of BDNF the percentage of calbindin-positive cells was higher (p = 0.01; Student's t test) in E17 than in E13 cultures. The calbindin-positive neurons in the E13 cultures also may, to some extent, represent patch neurons that transiently express this protein (Liu and Graybiel, 1992
NT-3 and NT-4/5 appear to act on the same subset of cells as does BDNF
On the basis of an analysis of BDNF
/
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Figure 6. NT-3 and NT-4/5, alone or in combination with BDNF, increase the number of DARPP-32-positive neurons to the same extent as does BDNF alone in both E13- and E17-derived cultures after 7 DIV. When used individually, growth factor concentrations were 100 ng/ml. In All, which contained BDNF, NT-3, and NT-4/5, the concentration of each neurotrophin was 10 ng/ml in E17, and 25 ng/ml in E13. All values are significant relative to control at p <0.001, except for E13-derived cultures in all neurotrophins at 7 DIV (p < 0.01).
In situ hybridization studies have demonstrated the presence of both trkB and trkC transcripts in the striatum (Ernfors et al., 1992
BDNF regulates ARPP-21 in vivo
We have established previously that DARPP-32 and ARPP-21 mRNAs are transcribed coordinately in most MSNs (Gustafson et al., 1992
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Figure 7. ARPP-21 expression is decreased in BDNF
DISCUSSION
We demonstrate that in vitro maturation of a large subset of striatal medium-sized spiny neurons, as defined by the expression of the DARPP-32, ARPP-21, and calbindin phenotype, requires neurotrophins. DARPP-32 and ARPP-21 transcription is initiated only in postmitotic, postmigrational MSNs (Foster et al., 1988
Recognizing that an in vivo versus in vitro comparison is not entirely accurate, we performed calculations to generate predictions of cell-type contents depending on the age of the embryo source of neurons. The striatum is composed of two neuronal compartments, the patch (or striosomes) and matrix (Graybiel, 1990
Our results differ significantly from other published data in which the percentage of DARPP-32-positive neurons in BDNF-treated rat LGE-derived neurons (mitotic and postmitotic) never exceeded 5% (Nakao et al., 1994a
Are the in vitro results of this study consistent with the in vivo observations? In mice with a targeted deletion of the BDNF gene, there is almost no detectable striatal calbindin (Jones et al., 1994
This study further highlights the heterogeneity of the MSN population: not only is there a multitude of MSN subtypes, but the same gene may be regulated differentially. There is a subset of MSNs that manifest the DARPP-32 phenotype in the absence of BDNF, and our data further suggest that there is another subset of MSNs that are DARPP-32-negative even in the presence of BDNF. It is highly likely that there are factors other than those in the neurotrophin family that regulate MSN maturation. For example, D2 and D1 receptor expression is highly responsive to retinoids, and this regulation varies regionally within the striatum (Krezel et al., 1998
The origin of BDNF within the striatum remains controversial. Several studies have demonstrated the presence of BDNF mRNA in the striatum (Hofer et al., 1990
The molecular mechanism of DARPP-32 and ARPP-21 induction by BDNF also remains to be determined. The nuclear effectors that correlate best with trk-mediated transcription are CREB and c-fos (Segal and Greenberg, 1996
In addition to defining the role of BDNF in the differentiation of the medium-sized spiny neuron, this study introduces a culture system in which highly differentiated MSNs may be generated, maintained, and studied. It is now clear that expression of the GABAergic phenotype and profound morphological differentiation are insufficient criteria by which to label an LGE-derived neuron as a medium-sized spiny neuron. Currently, we are extending our analysis to delineate further the neuronal subtypes present in our cultures as determined by receptor and neuropeptide expression. These data are particularly pertinent to any attempts to use cultured MSNs for physiological studies and/or in vitro analyses of toxins and therapeutic agents and strategies.
FOOTNOTES Received Dec. 31, 1998; revised March 24, 1999; accepted April 14, 1999.
This study was supported by grants from the National Institute of Mental Health, Hereditary Disease Foundation, and Irma T. Hirschl Trust. We are indebted to Dr. Olga Polonskaia for technical assistance and to Dr. Suzana Petanceska for help with the preparation of figures.
Correspondence should be addressed to Dr. Michelle E. Ehrlich, The Nathan Kline Institute, 140 Old Orangeburg Road, Orangeburg, NY 10962.
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